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Sample GSM6675691 Query DataSets for GSM6675691
Status Public on Mar 08, 2024
Title Trehalose_t10_rep1
Sample type SRA
 
Source name respiring yeast
Organism Saccharomyces cerevisiae
Characteristics tissue: respiring yeast
genotype: BY4741(MATa his3[delta]1 leu2[delta]0 met15[delta]0 ura3[delta]0)
treatment: 10 min before Antimycin A (final 2 ug/ml) treatment
Treatment protocol For Antimycin A treatment, Antimycin A was added to a final 2 ug/ml to the medium and incubate for 0, 2 ,5, and 10 min. Cells were fast spined down for 15 seconds at 13,000 g in a tabletop microcentrifudge and flash-frozen in liquid nitrogen.
Growth protocol S. cerevisiae were grown in trehalose-grown medium at 30°C. Trehalose-containing medium includes 20 g/l trehalose (Sigma), 6.7 g/l YNB + (NH4)2SO4 (yeast nitrogen base without amino acids; Difco), amino-acid supplements at a final concentration of 100 mg/l. The medium was buffered at pH 4.8 by adding 14.6 g/l succinic acid and 6 g/l NaOH. Pre-cultures were grown overnight in 250 mL flasks and agitated at 150 rpm. The next day, pre-cultures were diluted to OD600 = 0.05 and grown until an OD600 of ~0.5 was reached.
Extracted molecule total RNA
Extraction protocol Total RNA was isolated by the standard phenol chloroform method and DNA was removed by DNase I treatment, as described in Zhang & Pelechano, 2021 (PMID:33870233 ) : The amount of RNA was quantified using a Nanodrop 2000 Spectrophotometer (Thermo Scientific) and RNA integrity was checked by agarose gel electrophoresis.
For HT5Pseq libraries construction, we used 6 μg of DNA-free total RNA. Samples were directly subjected to RNA ligation. The treated RNA samples were incubated with 100 μM RNA/RNA rP5_RND oligo (final 10 μM) 2h at 25°C with 10 Units of T4 RNA ligase 1 (NEB). Ligated RNA was purified with RNAClean XP (Beckman Coulter), according to the manufacturer’s instructions. RNA was reverse transcribed with Superscript II (Life Technologies) and primed with Illumina PE2 compatible oligos containing random hexamers (20 μM) and oligo-dT (0.05 μM). Reverse transcription reaction was incubated for 10 min at 25°C, 50 min at 42°C and heat inactivation for 15 min at 70°C. To deplete RNA in RNA/cDNA hybrid after reverse transcription, we used sodium hydroxide (40 mM) for incubation 20 min at 65°C and then neutralized with Tris-HCl, pH =7.0 (40 mM). For DSN (Duplex-specific nuclease) based rRNA depletion, we used a mixture of probes targeted the 18S rDNA, 25S rDNA and 5.8S rDNA. The probes were designed to occupy the whole ribosomal RNA regions with consecutive 25-30nt long unmodified DNA oligos. The hybridization of probes (2 μM each) with cDNAs were incubated at 68 °C for 2 minutes before adding pre-warmed DSN buffer mix with 1 Units of DSN enzyme (Evrogen). The reaction then performed at 68 °C for 20 minutes. To inactive DSN enzyme, we added 2X DSN stop solution and incubate 10 min at 68 °C. The final PCR amplification was used 2X Phusion High-Fidelity PCR Master Mix with HF Buffer (NEB) and final 0.1 μM of PE1.0 and corresponding multiplex PE2.0_MTX . The program followed this: 30s 98°C; 15 cycles (20s 98°C; 30s 65°C; 30s 72°C); 7min 72°C. Libraries were size selected using 0.7x-0.9x (v/v) AMpure XP beads (Beckman Coulter) to final 200-500 bp and sequenced by NextSeq 2000 using 55 sequencing cycles for Read 1. 5PSeq methods was performed as previously described (PMID: 26820793). 6µg of total RNA was used as input. In brief a RNA oligo (rP5_RND) containing an Illumina adaptor and unique molecular identifiers (UMI) was ligated to the intermediates of mRNA co-translation degradation (5’P). Ribosomal RNA was depleted using Ribo-Zero Magnetic Gold Kit (Illumina).Libraries were PCR amplified (15 cycles). Ampure beads size selected libraries with an average length of 400 nt were sent for sequencing (llumina NextSeq 2000 instrument).
 
Library strategy OTHER
Library source transcriptomic
Library selection other
Instrument model NextSeq 2000
 
Data processing Base-calling was done using bcl2fastq v2.20.0.422 and for demultiplex, we allowed one mismatch in index1 and one mismatch in index2
For HT-5Pseq data, HT-5Pseq reads were trimmed 3’-sequecing adapter using cutadapt V1.16. The 8-nt random barcodes on the 5’ ends of reads were extracted and added to the header of fastq file as the UMI using UMItools (v0.5.4). Reads were mapped to the reference genome (SGD R64-1-1 for S. cerevisiae genome by star/2.7.9a with the parameter --alignEndsType Extend5pOfRead1 to exclude soft-clipped bases on the 5’ end. Duplicated 5’ends of read introduced by PCR during library preparation were removed based on random barcodes sequences using UMItools (v0.5.4).
For The distribution of nucleotide position of 5’ends were performed using Fivepseq package (PMID: 33575643), including relative to start, stop codon and codon specific pausing. Specifically, the unique 5’mRNA reads in biological samples were summed up and normalized to reads per million (rpm). Then the relative position of 5’mRNA reads to all codons of all ORF were summed at each position. The metagene plot was showed as the sum value versus the relative distance from respective codon.
Assembly: Saccharomyces cerevisiae R64-1-1
Supplementary files format and content: Bedgraph files for UMI collapsed reads for positive and negative strand. Reads were collapsed to the first 5´nucleotide.
Library strategy: 5PSeq
 
Submission date Oct 25, 2022
Last update date Mar 08, 2024
Contact name Vicent Pelechano
E-mail(s) vicente.pelechano.garcia@ki.se
Organization name ScilifeLab - Karolinska Institutet
Department MTC
Street address Nobels väg 16
City Solna
ZIP/Postal code SE-17177
Country Sweden
 
Platform ID GPL31112
Series (1)
GSE216524 Analysing the effect of cellular energy levels on codon-specific ribosome occupancy in vivo
Relations
BioSample SAMN31439225
SRA SRX18014600

Supplementary file Size Download File type/resource
GSM6675691_Trehalose_t10_1_S5_negative.bedGraph.gz 3.3 Mb (ftp)(http) BEDGRAPH
GSM6675691_Trehalose_t10_1_S5_positive.bedGraph.gz 3.3 Mb (ftp)(http) BEDGRAPH
SRA Run SelectorHelp
Raw data are available in SRA
Processed data provided as supplementary file

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